Mechanisms of vapor‐phase antibacterial action of essential oil from Cinnamomum camphora var. linaloofera Fujita against Escherichia coli

Abstract The purpose of this study was to investigate antibacterial activity of essential oil from Cinnamomum camphora var. linaloofera Fujita (EOL) at vapor phase and its mechanism of bactericidal action against Escherichia coli. Results showed that the vapor‐phase EOL had significant antibacterial activity with a minimum inhibitory concentration (MIC) and minimum bactericidal concentration (MBC) of 200 μl/L. Further analyses showed that treatment of E. coli with vapor‐phase EOL resulted in partial degradation of cell membrane, increased membrane permeability, leakage of cytoplasm materials, and prominent distortion and shrinkage of bacterial cells. FTIR showed that EOL altered bacterial protein secondary and tertiary structures. GC/MS analysis showed that the components of vapor‐phase EOL included linalool (69.94%), camphor (10.90%), nerolidol (10.92%), and safrole (8.24%), of which linalool had bactericidal activity. Quantum chemical analysis suggested that the antibacterial reactive center of linalool was oxygen atom (O10) which transferred electrons during antibacterial action by the donation of electrons.

Further analyses showed that treatment of E. coli with vapor-phase EOL resulted in partial degradation of cell membrane, increased membrane permeability, leakage of cytoplasm materials, and prominent distortion and shrinkage of bacterial cells.
FTIR showed that EOL altered bacterial protein secondary and tertiary structures.
GC/MS analysis showed that the components of vapor-phase EOL included linalool (69.94%), camphor (10.90%), nerolidol (10.92%), and safrole (8.24%), of which linalool had bactericidal activity. Quantum chemical analysis suggested that the antibacterial reactive center of linalool was oxygen atom (O 10 ) which transferred electrons during antibacterial action by the donation of electrons.

K E Y W O R D S
antibacterial mechanism, essential oil, linaloofera fujita, vapor-phase antimicrobial activity 2008; Zhang et al., 2019). It has been shown that linalool has antimicrobial effects on the common bacteria and respiratory pathogens in air (Cox et al., 2000;Sato, Krist, & Buchbauer, 2007;Wang et al., 2019;Yamaguchi, Inouye, & Takizawa, 2001). However, the vapor-phase antibacterial activity and its mechanism of EOL have not been studied. Escherichia coli is the most famous bacterium in human and animal intestine and the most widely and deeply studied bacterium in modern biology, the conclusion from E. coli by the methods of molecular biology can be used for the study of other creatures, so it is often used widely in scientific research as model microorganism. In this study, we elucidated the vapor-phase antibacterial mechanisms of EOL by investigating microscopic structure, membrane permeability, and biological macromolecular structural changes of E. coli. We also identified the antibacterial active center of the vapor-phase EOL by quantum chemical analysis.

| Experimental materials
Essential oils including linaloe wood oil, litsea cubeba oil, clove oil, cassia oil, star-anise oil, rosemary oil, mentha arvensis oil, eucalyptus oil, tea tree oil, orange oil, marjoram oil, and clary sage oil were provided by Guangzhou Baihua Spice Co., Ltd. Linalool, camphor, nerolidol, and safrole were provided by Guangzhou Guangyi Spice Co., Ltd. Nutrient agar and buffered peptone were purchased from Guangdong Huankai Microbial Science and Technology Co., Ltd. All other reagents were of analytical grade.

| Experimental microbe
Escherichia coli ATCC 25922 was provided by Inspection and Quarantine Technology Center of Guangdong Entry-Exit Inspection and Quarantine Bureau. The stock culture of E. coli was maintained on nutrient agar slopes at 4°C and subcultured every other week.
Bacterial suspension preparation: Strain was activated in nutrient broth for 24 hr and streaked onto nutrient agar plate. Single colony was picked to make bacterial suspension at the concentration of 1.5 × 10 8 CFU/ml (0.5 McFarland units).

| Treatment of Escherichia.coli with vaporphase EOL
Escherichia.coli was treated with EOL as described previously by Lopez et al (Goñi et al., 2009). Briefly, 100 μl bacterial suspension (0.5 McFarland units) was evenly spread on nutrient agar plates.
Appropriate amount of EOL was added to the center of the cover of Petri dish. Petri dishes were cultured invertedly at 37°C for 24 hr after sealing with parafilm and forming gas atmosphere of essential oils by heating covers with water bath.

| Determination of MIC and MBC of vaporphase EOL
MIC was measured by determining the lowest concentration of EOL that can inhibit the visible bacterial growth, while MBC was measured by determining the lowest concentration of EOL that can kill bacteria. EOL-treated plates without bacterial growth were exchanged with a different cover to remove the essential oil vapor and continued to culture at 37°C for 24 hr. The lowest concentration of EOL corresponding to the plates with bacterial growth represents MIC, and the lowest concentration without bacterial growth represents MBC.

| Crystal violet assay
Crystal violet assay was performed as described previously (Devi et al., 2010). Briefly, bacteria were collected from plates and dispersed into 8 ml of crystal violet (10 μg/ml in PBS) solution. After incubation at 37°C for 10 min, bacterial suspension was centrifuged at 4°C for 15 min (7,104 g). Optical density at 590 nm (OD 590 ) was measured for the supernatant using a spectropho-

| Conductivity test
The Bacteria was treated by linaloe wood oil at various concentrations (100-800 μl/L) for different time (0.5-3.5 hr) in the culture plate. The treated bacteria were collected by washing the plate using 5 ml sterile water. After the suspension adjusted to 7.0 McFarland units, the conductivity was measured using turbidimeter.

| Electronic microscopic analysis
Bacteria were collected from the plate, fixed, and observed under a scanning electron microscope (SEM) and a transmission electron microscope (TEM) as described previously (Chen et al., 2015(Chen et al., , 2016 Tyagi & Malik, 2010).
The baseline was corrected, and then, deconvolution was performed using Gaussian. Subsequently, the second derivative was performed for the curve fitting and minimization of the residuals. The content of the secondary structure was calculated according to the peak area.

| Fluorescence spectroscopy
Bacteria were collected from the plates using 10 ml of PBS (0.05 mol/L) and proceeded with fluorescence spectroscopic analysis as described previously (Pinotsi et al., 2016;Wachsmuth et al., 2015).

| GC/MS analysis
Gas chromatograph was performed using Agilent HP6890 equipped with DB-17MS silica-capillary column (30 m × 0.25 mm, 0.25 μm film thickness, Agilent). The injector temperature was 250°C, the carrier gas was helium of high purity, carrier gas flow rate was 1.0 ml/min, column temperature was increased from 50 to 280°C, the solvent was delayed for 2.15 min, the injection volume was 0.2 μl, and the split ratio was 1:50. Agilent 5,973 was used for MS analysis. The MS interface temperature was 250°C, ionization mode was EI, the electron energy was 70 eV, the ion source temperature was 230°C, and the scanning range was 20-550 m/z. Solid-phase microextraction (SPME) was performed with polydimethylsiloxane (PMDS, 100 μm) fibers for 24 hr at room temperature. Chemical composition of the essential oils was identified by NBS75K and WILEY275 on mass spectrometry data.

| Quantum chemical analysis
All quantum chemical parameters were calculated by Material Studio 5.5. Density functional theory (DFT) (B3LYP/6-31G(d)) was used as the model and calculated by high-performance computer cluster platform (HP DL5800) in Guangdong University of Technology.

| Comparison of the vapor-phase antibacterial activity between EOL and other essential oils
MICs and MBCs for different essential oils were determined ( Table 1).
The results showed that antibacterial activity of EOL and tea tree oil was much higher than that of other essential oils. A large number of studies have shown that tea tree oil has antibacterial activity (Pérez-Rosés, Risco, Vila, Peñalver, & Cañigueral, 2015), but little is known on the antibacterial activity of EOL.

| Effect of vapor-phase EOL treatment on the permeability of Escherichia.coli
Bactericidal activity, absorption rate of crystal violet, and conductivity were increased with the increases of the vapor-phase EOL concentration ( Figure 1). However, when vapor-phase EOL concentration was over 200 μl/L, bactericidal activity, absorption rate of crystal violet, and conductivity were not increased significantly (Figure 1).
Bactericidal activity reached 100% after 30 min treatment and further extension of treatment did not enhance its bactericidal activity significantly. In contrast, absorption rate of crystal violet and conductivity

| Effect of vapor-phase EOL treatment on the ultrastructure of Escherichia.coli
Normal E. coli has a typical short rod or cylindrical shape with full body and smooth surface (Figure 2A). After treatment with vaporphase EOL, bacterial surface became shrunken and shriveled.
Further TEM analysis showed that normal E. coli had an integral cell wall and membrane structure with evenly distributed cytoplasm ( Figure 2B). After treatment with vapor-phase EOL, cell wall structure remained intact, but the cell membrane appeared partial rupture, leading to the leakage of the intracytoplasmic materials. In addition, cell membrane and cell wall were separated and the cytoplasm became unevenly distributed ( Figure 2C). These results suggested that EOL treatment disrupted the cell membrane structure, leading to the increase of cell permeability, leakage of intracellular substances, and shrinkage of bacterial shape.

| Effect of vapor-phase EOL treatment on the tertiary structure of bacterial protein
The leading to the increase of fluorescence intensity. However, when EOL concentration is too high (>200 μl/L), spreaded protein molecules become curled and folded, which results in the internalization of the exposed chromophores.

| Effect of vapor-phase EOL treatment on the secondary structure of bacterial protein
The amide I (1600-1700 cm −1 region) in the infrared spectrum is mainly the absorption of stretch vibration of C = O bond in the amino acids and it reflects α-helix, β-sheet, β-turn, and random coil conformation ( Figure 4A). To gain more information, we utilized second derivative and deconvolution to analyze the amide I region and obtained 9 subpeaks after curve fitting ( Figure 4B). 1682-1700 cm −1 are β-sheet, the peak at 1646-1664 cm −1 is αhelix, the peak at 1664-1681 cm −1 is random coil, and the peak at 1664-1681 cm −1 is β-turn. The effect of EOL treatment on each secondary structure was shown in Figure 4C. The results showed that vapor-phase EOL treatment greatly reduced the content of αhelix and increased the content of β-sheet. These results indicate that EOL alters the intramolecular hydrogen bond arrangement and changes the α-helix of peptide into linear structure, which leads to the alteration of bacterial protein secondary structure.
However, β-turn and random coil content was not significantly affected by EOL treatment ( Figure 4C).

| Antibacterial activity of components in the vapor-phase EOL
GC/MS analysis identified 45 main chemical components accounting for 99.53% of EOL ( Figure 5A). However, only four components F I G U R E 3 Effect of vapor-phase EOL on the protein fluorescent intensity F I G U R E 4 Effect of vapor-phase EOL treatment on the secondary structure of bacterial protein F I G U R E 5 GC/MS analysis of EOL and its vapor phase (linalool, camphor, nerolidol, and safrole) were identified in the vapor-phase EOL ( Figure 5B and Table 2). MICs and MBCs for components of vapor-phase EOL were shown in Table 3. MIC and MBC of vapor-phase EOL were similar to those of linalool, while there was no antibacterial activity for camphor, nerolidol, and safrole at the highest experimental concentration (3,000 μl/L). These results suggest that the antibacterial activity of vapor-phase EOL is mainly derived from linalool.

| Quantum chemical analysis of linalool
Studies have shown that the antibacterial activity of a substance is closely correlated to its energy of the highest occupied molecular orbit (E HOMO ) and the energy of the lowest unoccupied molecular orbit (E LUMO ) (18 Therefore, the main electron transfer occurred during antibacterial action of linalool is the donation of electron. Linalool atom numbering was shown in Figure 6, and the electron density of each atom was shown in Fukui function of linalool was calculated by Mulliken algorithm and the electrophilicity, nucleophilicity, and free radical affinity were obtained ( Table 6). The results showed that hydroxy group with O 10 atom has a strong electrophilicity and free radical affinity, which is very important for linalool to disarrange the intramolecular hydrogen bond arrangement of protein during antibacterial process. These results further confirmed that O 10 is the reactive center of antibacterial activity of linalool.

ACK N OWLED G M ENTS
We are grateful for the financial and moral assistance pro-

CO N FLI C T O F I NTE R E S T
Authors declare they have no conflicts of interest.

E TH I C A L A PPROVA L
This article does not contain any studies with human or animal subjects performed by any of the authors.